Bio-Rad Sub-Cell® Model 192 Cell User Manual

Section 5
Troubleshooting

Symptoms

Probable Causes

Solutions

Slanted lanes (bands)

Curved line or distortion of
lanes (bands)

Differential relative mobilities

Curved bands, smiles

Ragged bands

Band smearing and streaking

Bands sharp but too few bands
seem

High MW bands sharp/Low MW
bands smeared

Gels crack

• Gel not fully solidified.

• Comb warped or at an angle.

• Bubbles in sample wells.

• Sample spilled out of wells.

• Unit not leveled.

• Gel floated or slid off tray.

• Sample overload.

• Temperature or pH buffer

gradients

• Sample density incorrect.

• Sample well deformed.

• Excessive power or heating.

• Agarose has improper endos-

mosis (-m

r

).

• Salt concentration in sample

too high.

• Excessive power and heating.

• Sample spilled out of well.

• Incomplete digest, nuclease

contamination, bad enzyme.

• Sample wells cast through the

gel. Sample leaks along bot-
tom of running surface.

• Sample overload.

• Too high gel percentage.

• Incomplete digest.

• Gel percentage too low.

• Too high voltage gradient

especially with low melting
temperature agarose or low gel
strength gels.

• Let gel solidify for at least

30-60 minutes.

• Check alignment of comb.

• Remove bubbles prior to

electrophoresis.

• Samples should have proper

density. Apply carefully.

• Level unit. Place on steady

work bench.

• Recirculate at a rate of

300-500 ml/min.

• Reduce the amount of sample

loaded.

• Reduce load.
• Add more buffer.
• Recirculate buffer.

• See sample application

instructions.

• Carefully remove comb, espe-

cially from soft gels. Be sure
gel has solidified. Cooling soft
gels aids in comb removal.
Add buffer to help lubricate
removal of the comb.

• Reduce voltage. See elec-

trophoresis instructions.

• Consult Bio-Rad about

agarose.

• Reduce salt concentration to

≤

0.1 M.

• Reduce voltage. See elec-

trophoresis instructions

• Take care in applying sample.

Increase gel thickness for large
sample volumes.

• Heat sample. Check enzyme

activity. Digest sample further.

• Comb should be placed 1 to

2 mm above the base of the run-
ning surface. Add buffer to help
lubricate removal of the comb.

• Dilute sample.

• Lower gel percentage.

• Check enzyme activity, digest

further.

• Increase gel percentage.
• Switch to polyacrylamide.

• Reduce voltage. Run gel at

lower temperature.

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